WO1995021924A1 - Expression of the glucose oxidase gene in transgenic organisms - Google Patents

Abstract

A genetic construct for use in production of transgenic plants and other organisms with reduced susceptibility or increased resistance to pests or diseases comprises an isolated nucleotide sequence encoding, or complementary to a sequence encoding, the glucose oxidase enzyme or a functional derivative thereof, the nucleotide being operably linked to a promoter capable of expression in the host organism.

Description

EXPRESSION OF THE GLUCOSE OXIDASE GENE IN TRANSGENIC ORGANISMS.

FIELD OF THE INVENTION.

This invention relates to the production of the transgenic organisms (including for example, plants, microbes and viruses) that express a glucose oxidase gene whose gene product is toxic to economically important pests and diseases of crops. Transgenic plants in accordance with this invention can be sold as improved varieties, whilst transgenic microbes and viruses can be used as biopesticides or as seed coatings or inoculums for soil incorporation.

BACKGROUND OF THE INVENTION. Production of most crop species is limited by the ravages of pests and diseases. Considerable expense is involved in the protection of crops from these organisms and many current conventional breeding programs are directed at increasing host plant resistance to a variety of invertebrate pests and fungal or viral diseases. Traditional sources of host plant resistance are limited to the same species or species closely related to the crop, but with the advent of genetic engineering novel sources of resistance outside the crop genera are being accessed. Two classic examples are the insecticidal protein genes from Bacillus thuringiensis active against a multitude of insect species (Perla et al. , 1990) and the viral coat protein genes that confer tolerance to a variety of related viral diseases (Powell etal. , 1986). Transgenic plants expressing these genes have enormous potential markets once the regulatory hurdles are overcome for their large scale release into agriculture.

New sources of host plant resistance are being sought from a variety of sources, and work leading to the present invention has led to the isolation and characterisation of a glucose oxidase gene from the fungus Talaromyces flavus that has potential for the control of both fungal diseases and arthropod pests when expressed in transgenic crop plants. The particular examples investigated to date are for the control of the cotton pathogen, Verticilliυm dahliae , the causal agent of verticillium wilt disease, and for the control of Helicoverpa spp. which are economically important Lepidopteran pests of cotton and most summer crops. Use of the glucose oxidase gene for the control of other fungal diseases or pests such as nematodes, mites, aphids, whiteflies, jassids or mirids which are susceptible to hydrogen peroxide produced by glucose oxidase activity is also possible.

Verticillium Wilt as a Cotton Pathogen

Verticillium wilt is a wide-spread disease which affects many different plant species. It is caused by the soil fungus Verticillium dahliae (Leb.), an imperfect fungus first isolated from diseased dahlias in 1913 (Muller, 1928). Isolates of the species vary widely in both morphology and pathogenicity but all produce small, hard black structures called microsclerotia. These structures are composed of melanized cells which store many nutrients and are the means by which V. dahliae survives in the soil.

V. dahliae does not grow saprophytically through the soil, but conidia and microsclerotia germinate in soil if root exudate from desirable plant species are present. The mycelium then invades the plant, entering through the cap of the root region of elongation, root hairs or lower hypercotyl region. In all cases both intercellular and intracellular invasion occurs. In "susceptible" hosts, the fungus successfully penetrates the vascular system of the plant. Here hyphal multiplication occurs and conidiospores are generated which then travel upwards through the xylem thus spreading the fungus rapidly through the vascular system of the plant.

Once spread throughout the vascular system the main effect of the pathogen is to disrupt the passage of water through the stem. This may be attributed to the physical presence of the mycelium of the pathogen, the development of tyloses that block the xylem or to gummosis within the vessels. Further xylem occlusion is caused by high molecular weight polysaccharides produced by the pathogen or cleaved from the plant walls by hydrolytic enzymes. Together this can result in a 40 to 60-fold increase in the resistance of the stem to water flow; thus the characteristic wilting of leaves occurs (Ayer and Racok, 1990).

In cotton more obvious symptoms include a yellowing of lower leaves, vascular discolouration and stunting of plant growth. Some V. dahliae isolates also cause severe defoliation of the cotton plant. On the basis of heterokaryon incompatibility tests these isolates fall into a separate group from the less severe, non-defoliating isolates (Puhalla, 1979). All Australian isolates so far examined belong to the less severe, non-defoliating group, however they are still capable of causing a significant reduction in lint yield.

Controlling verticillium wilt in cotton in Australia has frequently been a problem, particularly in the cooler growing regions (New South Wales and Southern Queensland) where cooler, wetter seasons promote more vigorous fungal growth. The microsclerotia produced are resistant to many soil fumigants and remain viable in the soil for many years. Crop rotation is also not a satisfactory control measure because of the wide host range of the fungus. No natural resistance to Verticillium has been identified in cotton, any natural tolerance that has been found is being exploited by the breeders.

Biological control of the pathogen with other microbes is a possible solution. Marios et al. (1982) investigated the potential of over 30 different soil fungi to control verticillium wilt development in eggplant under field conditions. An isolate of Talaromyces flavus was identified that reduced disease symptoms by approximately 70% in two separate field situations. Trials have shown that T. flavus is able to occupy the rhizosphere of Australian cotton. Further trials will need to be done to determine if this naturally occurring strain or improved engineered strains can control verticillium wilt. However, even if successful, T. flavus itself may not be a suitable control agent as large scale seeding of soil in which cotton is to be grown may be impractical and other microbes that live in close association with the cotton plant may be more effective delivery systems.

Helicoverpa spp. are serious pests of cotton and other summer crops. Helicoverpa armigera and H. puctigera are two of the most economically important insect pests in many cropping systems in Australia (Fitt, 1989). Their larvae cause considerable damage in crops such as cotton and their control requires the application of vast amounts of chemical pesticides. Many of these pesticides are becoming ineffective due to the development of resistance by the insects and sources of host plant resistance in the crop would be extremely valuable, both economically and environmentally.

Adult moths lay their eggs singly, generally on the young growing tips of the plant. When the neonates emerge they feed on the egg case and then migrate to the young flower buds (squares) and begin to graze. A single larvae may visit several flower buds rather than staying on one square for extended periods of time. Relatively small amounts of feeding damage cause flower abortion and hence the economic threshold for larvae on plants is relatively low. As little as one larvae per metre of cotton row can have a significant effect on yield, so relatively low infestations must be sprayed to control the insect. As indicated below, glucose oxidase is toxic to these caterpillars when incorporated into synthetic diets containing a source of glucose and so may be a useful gene to express in young cotton tissues such as leaves and squares.

Talaromyces flavus is a glucose oxidase secreting ascomycete.

Talaromyces flavus (Klocker) Stolk and Samson (anamorph Penicillium dangeardii Pitt, usually reported as P. vermiculatum Dangeard) is the most common species of its genus. This ascomycete is frequently isolated from soil, although it may also occur in other organic substrates. It is widely distributed around the world but is more commonly found in warmer regions. It has been reported as a potential biocontrol agent for several other fungal pathogens, Rhizoctonia solani (Boosalis, 1956) and Sclerotinia sclerotiorum (McLaren et al., 1986).

In the above cases, T. flavus controls the pathogens by mycoparasitism, that is T. flavus parasitises its fungal host for nutrient gain. Infection studies of S. sclerotiorum and R. solani have shown T. flavus coils around the host developing hyphal branches which then penetrate the host's cells. Deterioration of the cytoplasm follows with the infected cells eventually collapsing, although the cell walls remain intact. Transmission electron micrographs of V. dahliae microsclerotia parasitised by T. flavus have similarly shown cell invasion and lysis taking place only at the contact sites between the host's cells and T. flavus hyphal tips (Madi et al., 1989).

The mechanisms involved in the parasitic interactions are unclear. However Fravel et al., (1987) found T. flavus secreted a metabolite into liquid medium which in the presence of glucose was toxic to microsclerotia and inhibited radial growth of Verticillium mycelia. The active component was subsequently identified as glucose oxidase secreted from fungal hyphae (Kim et al., 1988). This enzyme has now been shown to inhibit other fungi including several of the Pythium species, Rhyzoctonia solani and Sclerotinia minor (Kim et al., 1990^{a b}).

Glucose oxidase leads to the production of hydrogen peroxide, (H₂0₂) as a by-product of glucose oxidation:

Glucose + H₂0+0₂ Glucose Gluconic + Hydrogen > Acid Peroxide

Oxidase

When added to growth media, hydrogen peroxide inhibited microsclerotial germination and mycelial growth. The other reaction components, glucose oxidase (no glucose present), gluconic acid and glucose did not cause inhibition

(Kim et al., 1988). Thus the antifungal activity of glucose oxidase is due to the hydrogen peroxide it produces. However when the peroxide scavenger catalase was added to the culture filtrate of T. flavus there was only a loss of 50% of its toxic activity towards V. dahliae (Madi et al., 1989). Thus T. flavus may produce other agents toxic to V. dahliae. T. flavus has been found to excrete a range of lytic enzymes including cellulases, /?-1-3-glucanases and chitinase. Therefore the antagonistic activity of T. flavus towards V. dahliae may be due to a combined effect of lytic enzymes and toxic metabolites. The glucose oxidase may act by inhibiting the Verticillium and thus predispose the hyphae to infection before contact occurs.

Glucose oxidase the active agent in the antagonism by T. flavus of V. dahliae.

The enzyme glucose oxidase is known to be produced by different species of Aspergillus and Penicillium, by Talaromyces flavus and by the basidiomycete Phanerochaete chryosporium, (white rot fungus). In P. chryosporium (found in wood), the hydrogen peroxide produced is required by a ligninase enzyme for the degradation of lignin. In the other fungi little is known about the enzyme's biological function. They may produce enzymes which utilise hydrogen peroxide as P. chryosporium does. In this case the enzyme's ability to inhibit various other soil fungi may be a secondary effect, however it would benefit the host in certain competition situations.

Glucose oxidase has been purified from each of the four fungal genera known to produce it. In all cases, the enzyme is a dimeric flavoprotein with an optimum pH of 5.0. The most distinct enzyme is that of P. chryosporium. Unlike the others it is not glycosylated and although glucose is its primary substrate it is also induced to a smaller degree by sorbose, xylose and maltose (33, 13 and 7% respectively) (Kelly and Reddy, 1986). The other enzymes are highly specific for ?-D-Glucose.

Glucose oxidase from T. flavus has a relative molecular weight of 164,000 (subunit molecular weight 71,000) (Kim et al., 1990). This is similar to that of Penicillium amakienase (150,000) and Aspergillus niger (152,000), (Nakamura and Fujiki, 1968). It is stable from pH 3.0 to 7.0, unlike A. niger which is restricted to pH 4.5 to 6.5. Six isozymes with pi values of 4.40 to 4.55 have been detected. These are thought to be due to differences in sugar residues as opposed to differences in amino acid sequence. It has a relatively low affinity for glucose with a Km for /?-D-glucose of 10.9 mM. This is however a higher affinity than that of A niger which has a Km for ?-D-glucose of 27 mM.

The gene for glucose oxidase from A. niger has been cloned by several groups (Kriechbaum etal., 1989, Frederick et al., 1990, Whittington etal., 1990). The structural gene consists of 1815 bp encoding 605 amino acid residues. The mature protein contains 583 amino acids, the difference being due to 22 amino acids which comprise the secretion signal presequence. No introns were present in the coding region. The gene has been introduced into Aspergillus nidulans and the yeast Saccharomyces cerevisiae where it provided the novel capacity to produce glucose oxidase. It has also been reintroduced into A. niger where increased copy number increased glucose oxidase production.

ln the past, biological control of pests and diseases has focussed on natural biocontrol agents such as antagonistic bacteria and fungi or viruses. It has now been found that the effectiveness of these agents can be enhanced if they are engineered to express the glucose oxidase activity. The present invention therefore includes the use of other vectors for delivering the glucose oxidase activity to the pest or pathogen, such as root or leaf colonising micro¬ organisms which could be beneficial bacteria or fungi that live around the plant and that could exert their effects on plant pests in the rhizosphere or phylloplane or, for example, insect specific viruses that could be sprayed onto the plants.

SUMMARY OF THE INVENTION.

The present invention provides a genetic construct comprising an isolated nucleotide sequence encoding, or complementary to a sequence encoding, the enzyme glucose oxidase or a functional derivative of the enzyme, said

nucleotide sequence being operably linked to a promoter capable of expression in a host organism.

By the term "isolated nucleotide sequence" is meant a genetic sequence in a non-naturally-occurring condition. Generally, this means isolated away from its natural state or synthesized or derived in a non-naturally-occurring environment. More specifically, it includes nucleic acid molecules formed or maintained in vitro, including genomic DNA fragments, recombinant or synthetic molecules and nucleic acids in combination with heterologous nucleic acids.

Any suitable promoter may be incorporated in the genetic construct of the present invention. By way of example only, the promoter may be the promoter of the 35S transcript of cauliflower mosaic virus or the tobacco root-specific promoter pTOBRB7.

The terms "genetic sequence" and "nucleotide sequence" are used herein in their most general sense and encompass any contiguous series of nucleotide bases specifying directly, or via a complementary series of bases, a sequence of amino acids in the enzyme glucose oxidase. Such a sequence of amino acids may constitute a full-length glucose oxidase, or an active truncated form thereof, or may correspond to a particular region such as an N-terminal, C-terminal or internal portion of the enzyme.

The genetic construct of the present invention may be introduced into a host organism such as a plant, bacterium or virus in order to provide the host organism with glucose oxidase activity, or elevate endogenous glucose oxidase activity, in the host organism. Reference herein to the elevation of glucose oxidase activity relates to an elevation in activity of up to 30% or more preferably of 30-50%, or even more preferably 50-75% or still more preferably 75% or greater above the normal endogenous or existing levels of glucose oxidase activity of the host organism. The nucleic acids of the genetic constructs of the present invention may be ribonucleic acid or deoxyribonucleic acids.single or double stranded and linear or covalently closed circular molecules. Preferably, the nucleotide sequence is cDNA. The present invention also extends to other nucleotide sequences which hybridize under low, preferably under medium and most preferably under high stringency conditions with the nucleotide sequence of the present invention and in particular to the sequence of nucleotides set forth in SEQ ID. NO:1 hereinafter or a part or region thereof. In its most preferred embodiment, the present invention extends to a genetic construct, having a nucleotide sequence set forth in SEQ ID. NO:1or to a construct having at least 40%, more preferably at least 45%, even more preferably at least 55%, still more preferably at least 65-70%, and yet even more preferably greater than 85% similarity at the level of nucleotide or amino acid sequence to at least one or more regions of the sequence set forth in SEQ ID. NO: 1 and wherein the construct encodes or is complementary to a sequence which encodes an amino acid sequence having glucose oxidase activity.

In this regard, the nucleic acid may include the naturally-occurring nucleotide sequence encoding glucose oxidase or it may contain single or multiple nucleotide substitutions, deletions and/or additions to said naturally- occurring sequence. The nucleic acid of the present invention or its complementary form may also encode a non-full length portion of this enzyme which retains the glucose oxidase activity.

The nucleotide sequence or its complementary form may encode the full- length glucose oxidase enzyme, or a functional derivative thereof. By "functional derivative" is meant any single or multiple amino acid substitution, deletion and/or addition relative to the naturally-occurring enzyme and which retains glucose oxidase activity.

Amino acid insertional derivatives of the glucose oxidase enzyme include amino and/or carboxyl terminal fusions as well as intra-sequence insertions of single or multiple amino acids. Insertional amino acid sequence variants are those in which one or more amino acid residues are introduced into a predetermined site in the protein although random insertion is also possible with suitable screening of the resulting product. Deletional variants are characterised by the removal of one or more amino acids from the sequence. Substitutional amino acid variants are those in which at least one residue in the sequence has been removed and a different residue inserted in its place. Typical substitutions are those made in accordance with Table 1 hereunder.

Where the glucose oxidase is derivatised by amino acid substitution, the amino acids are generally replaced by other amino acids having like properties, such as hydrophobicity, hydrophilicity, electronegativity, bulky side chains and the like. Amino acid substitutions are typically of single residues. Amino acid insertions will usually be in the order of about 1-10 amino acid residues and deletions will range from about 1-20 residues. Preferably, deletions or insertions are made in adjacent pairs, i.e. a deletion of two residues or insertion of two residues.

The amino acid variants referred to above may readily be made using peptide synthetic techniques well known in the art, such as solid phase peptide synthesis and the like, or by recombinant DNA manipulations. Techniques for making substitution mutations at predetermined sites in DNA having known or partially known sequence are well known and include, for example, M13 mutagenesis. The manipulation of DNA sequence to produce variant proteins which manifest as substitutional, insertional or deletional variants are conveniently described, for example, in Sambrook et al. (1989). TABLE 1 Suitable residues for amino acid substitutions.

Original Residue Exemplary Substitutions

Ala Ser

Arg Lys Asn Gin; His

Asp Glu

Cys Ser

Gin Asn

Glu Asp Gly Pro

His Asn; Gin lie Leu; Val

Leu lie; Val

Lys Arg; Gin; Glu Met Leu; lie

Phe Met; Leu; Tyr

Ser Thr

Thr Ser

Trp Tyr Tyr Trp; Phe

Val lie; Leu

Other examples of recombinant or synthetic mutants and derivatives of the glucose oxidase enzyme of the present invention include single or multiple substitutions, deletions and/or additions of any molecule associated with the enzyme such as carbohydrates, lipids and/or proteins or polypeptides.

The term "functional derivatives" also extends to any functional chemical equivalent of the glucose oxidase and also to any amino acid derivative described above. For convenience, reference to "glucose oxidase" herein includes reference to any mutants, derivatives, analogues, homologues or fragments thereof. The present invention is exemplified using an isolated nucleotide sequence derived from Talaromyces flavus as set forth in Table 2 (SEQ. ID No:1) since this represents the most convenient and preferred source of material to date. However, one skilled in the art will immediately appreciate that similar sequences can be isolated from any number of sources. All such nucleic acid sequences encoding directly or indirectly a glucose oxidase enzyme, regardless of their source, are encompassed by the present invention.

The genetic construct contemplated herein may exist in combination with a vector molecule, for example an expression-vector. The term "vector molecule" is used in its broadest sense to include any intermediate vehicle for the nucleic acid molecule, capable of facilitating transfer of the nucleic acid into a host organism and/or facilitating integration into the host genome. Where the host organism is a plant, the intermediate vehicle may, for example, be adapted for use in electroporation, microprojectile bombardment, Λgra acfera/m-mediated transfer or insertion via DNA or RNA viruses. The intermediate vehicle and/or the nucleic acid molecule contained therein may or may not need to be stably integrated into the plant genome. Such vector molecules may also replicate and/or express in prokaryotic cells. Preferably, the vector molecules or parts thereof are capable of integration into the host genome. The genetic construct may additionally contain a promoter sequence operably linked to, and capable of directing expression of, the nucleic acid molecule in the host organism. The nucleic acid molecule and promoter may also be introduced into the host organism by any number of means, such as those described above.

In another aspect, the present invention also provides a transgenic organism capable of expressing a cloned nucleotide sequence encoding the enzyme glucose oxidase or a functional derivative thereof. As described above, the transgenic organism is preferably a plant, for example a cotton plant, or a micro-organism or virus, particularly a root- or leaf-colonising micro-organism or an insect-specific virus. ln a preferred embodiment the cloned nucleotide sequence is the

Talaromyces flavus glucose oxidase gene as represented by the nucleotide sequence of SEQ ID. No:1 , however it will be understood that glucose oxidase genes from other organisms are also encompassed within the scope of the invention.

The invention therefore comprises the expression of the cloned T. flavus glucose oxidase gene or other sources of glucose oxidase genes in a transgenic organism, which may be either a plant or a virus or microbe that is brought into contact with a pest species, insect, other arthropod, nematode or disease causing microbe for the control of that pest or disease organism.

The invention may also include the expression of a second gene for the generation of the glucose required for the toxic effect exerted by the glucose oxidase enzyme.

In work leading to the present invention, the antifungal activity of T. flavus glucose oxidase in vitro has been demonstrated, as has the insecticidal activity of glucose oxidase in synthetic diets. The glucose oxidase gene from T. flavus has been cloned and sequenced, and the functionality of the cloned gene has been established by expression of the cloned glucose oxidase gene in a transgenic fungus originally lacking glucose oxidase activity, and by demonstration of in vitro fungal antagonism by this strain.

In addition, a number of genetic constructs have been made to express the

T. flavus glucose oxidase gene using standard cloning methods, and these constructs have been transformed into plants using known transformation vectors and protocols to obtain the expression of functional glucose oxidase in the transgenic plants. Transgenic plants expressing glucose oxidase were found to be more tolerant to fungal infection than control plants. Glucose oxidase can be expressed in transgenic plants.

The expression of the fungal glucose oxidase in transgenic plants poses a number of problems, not the least of which is that the enzyme may have some toxic side effects on the plant itself. The enzyme is excreted from the fungal cell and needs to be equipped with appropriate signals for secretion by plant cells. A number of gene constructs have been constructed to express the T. flavus gene both constitutively, tissue specifically and conditionally in transgenic plants. In initial experiments, tobacco (Nicotiana tabacum) was used as a recipient because of the long time frame for the generation of transgenic cotton. The different gene constructs were assembled by standard cloning methods (Sambrook et al., 1989), fused to a 3' end from nopaline synthase (NOS 3') and transformed into plants using the binary transformation vectors and protocols of An et al. (1985). The salient features are the type of promoter and the signal sequence at the N-terminal end of the translated glucose oxidase protein. Cellular targeting may be important for the effective expression of the fungal glucose oxidase in other species. It appears that the fungal signal peptide necessary for the excretion of the glucose oxidase protein in Talaromyces is not functional in plants as the native coding region was not expressed in transgenic tobacco tissues. The form of the signal peptide has many options but in one preferred form has the signal sequence from the carrot root extensin gene (Chen & Varner, 1985) and when introduced into transgenic tobacco this modified coding region did produce a functional glucose oxidase protein. The promoter may be any plant promoter resulting in high levels of expression of the introduced glucose oxidase gene. The promoters of the 35S transcript of cauliflower mosaic virus (Odell et al., 1985) or the tobacco root-specific promoter pTOBRB7 (Conkling et al., 1990) have been used, and both produced detectable levels of expression of the glucose oxidase gene in transgenic tobacco when assayed with the coupled peroxidase assay of Fiedurek et al., (1986).

Further features of the present invention will be apparent from the accompanying drawings. ln the drawings:

Figure 1 shows growth inhibition of Verticillium by culture filtrates from T. flavus. Verticillium growth was monitored by light scattering at 595 nm using an automated micro-titre plate scanner. Each well continued 200 μ\ of Potato Dextrose medium supplemented with culture filtrates from T.flavus 32908, T.flavus (var macrosporus) a non-glucose oxidase producer, a glucose oxidase positive transformant of var macrosporus or PD medium as a control. Each experiment contained approximately the same amount of glucose oxidase activity (approx. 1.5 μg).

Figure 2 shows hybridisation of A. niger glucose oxidase gene to genomic DNA digests at different stringencies. A: Autoradiograph of a Southern blot of BamH 1 digests of DNA hybridised with ³²P labelled A. niger glucose oxidase gene. Hybridisation performed at 37°C and filter washed with 1XSSC at room temperature. Lane 1 , T. flavus 26015 DNA; lane 2, T. flavus 32908 DNA; lane 3, A. niger 9029 DNA; lane 4, A. nidulans DNA; lane 5, Hind III digest of ³²P-labelled 1 DNA. Faint bands in lanes 1 and 2 are arrowed. B: Autoradiograph of a Southern blot of BamH 1 digested T. flavus 32908 DNA hybridised with the A. niger glucose oxidase gene. Hybridisation performed at 30°C and the filter washed with 2XSSC at room temperature. Lane 1 , T. flavus 32908 DNA; lane 2 Hind III digest of ³²P-labelled 1 DNA. The Hind III 1 size markers are shown in kilobases (kb).

Figure 3 is a schematic outline of glucose oxidase expression cassettes transformed into tobacco. Constructs contain the glucose oxidase gene fused in frame with the carrot root extensin signal peptide (A) or its own glucose oxidase signal peptide (B). Glucose oxidase was placed under control of either the carrot root extensin, TobRB7 or 35S promoter and the 3' end fused to the nopaline synthase (nos) terminator sequence from A. tumefaciens. All constructs were cointegrated into the EcoRI site of the binary vector pTAB5 in an indirect orientation to the selectable kanamycin resistance gene. Abbreviations: E, EcoRI; npt\\, neomycin phosphotransferase; LB, Left Border; RB, Right Border. Linear maps are not drawn to scale.

Figure 4 shows in vitro inhibition of R. solani growth. Either A. niger glucose oxidase or culture filtrate from T. flavus 32908 or GOH-1 were incorporated into growth medium and growth of R. solani monitored over 38 hours. The glucose oxidase concentration in media containing A. niger glucose oxidase and 7. flavus 32908 filtrate was 0.10 units/ml where one unit + that amount which oxidases 1.0 /mole ofyff-D glucose to D gluconic acid and H₂0₂ per minute at pH 5.1 and 25°C. Standard error was 10-17% of the values obtained (omitted from graph for the sake of clarity).

Figure 5 shows growth inhibition of R. solani in different amounts of T. flavus culture filtrate and different concentrations of A. niger glucose oxidase. The amount of glucose oxidase in the culture filtrate was determined by comparison to standard concentrations of A. niger glucose oxidase.

EXAMPLE 1 Fungal Strains Verticillium fungal isolates were obtained from Dr.S.AIIen, Agricultural

Research Station, Narrabri. The four isolates (#2, #13, #24, #34) were isolated from cotton in 1990 from farms in different areas.

Three Talaromyces flavus strains were obtained from Dr. J.Pitt, CSIRO Food Research. These three strains were:

FRR 2268 ex Brazilian passionfruit concentrate imported into Australia (var macrosporus) FR 2386 ex Australian passionfruit (var macrosporus) FRR 2417 ex soil, passionfruit farm, NSW North Coast (var macrosporus).

Two other T. flavus strains were obtained from the American Type Culture Collection (ATCC): ATCC 26015 ex wood, Japan.

ATCC 32908 ex soil, Japan.

The Aspergillus niger strain from which the glucose oxidase gene was cloned was also obtained from the ATCC: ATCC 9029 ex soil, USA.

An Aspergillus nidulans strain was obtained from Dr. M. Hynes, Melbourne University.

Demonstration of the production of glucose oxidase by Talaromyces flavus and inhibition of Verticillium growth.

Preliminary experiments were done to confirm that glucose oxidase was being produced by the T.flavus (var macrosporus) strains and that this was inhibitory in Australian V. dahliae isolates. Initial experiments were performed with the T. flavus strains obtained from Dr. J. Pitt. In each case, a spore suspension was transferred to liquid culture medium (potato dextrose + 8% glucose), this was maintained at 35° on a rotary shaker for 72 hours. The broth was filtered to remove mycelium and then incorporated 1 :1 into double strength Czapeck Dox solution agar. Control plates were made with uninoculated potato dextrose broth. Verticillium mycelial disks were transferred to the plates and radial growth of the developing colonies recorded every 2 days for 8 days. Similar experiments in liquid medium monitored hyphal growth monitored spectrophotometrically as light scattering. No significant reduction in V. dahliae growth was observed. Experiments were repeated using the ATCC T.flavus isolates. Both cultures proved inhibitory, 32908 more than 26015. This is presumably because 32908 secretes more glucose oxidase and/or less peroxidase scavengers. Inhibition for the 32908 strain is shown in Figure 1. Glucose oxidase production clearly varies between different isolates of Talaromyces and is not present in the macrosporus biotypes. It was also noted that some V. dahliae isolates were more susceptible to inhibition than others. ln order to determine that glucose oxidase was being produced, three different assay systems were used. Two indicator plates were developed for quantitative analysis. Both plates were composed of two layers, the bottom layer in both cases containing potato dextrose + 2.5% glucose. The top layer of the first plate contains various mineral salts and calcium carbonate. Gluconic acid produced as a product of glucose oxidase activity dissolves the calcium carbonate resulting in a clear ring around the fungus (Witteveen et al., 1990). The other indicator plate's top layer contains potassium iodide (Kl) and starch. Iodine is released from potassium iodide by glucose oxidase and this combines with the starch to form violet-blue zones (Fiedurek et al., 1986). Both ATCC T. flavus isolates scored positive in these plate assays while the macrosporus biotypes scored negative.

Quantitative analysis of enzyme activity was performed using a spectrophotometric method. This assays for the production of H₂0₂ using reduced O-Dianisidine and Horse Radish Peroxidase. Oxidised O-Dianisidine produced by the reaction is a red colour and can be measured at 400 nm on a spectrophotometer (Fiedurek et al., 1986).

/?-D-Glucose+0₂+H₂0 Glucose D-Gluconic Acid+H₂0₂ >

Oxidase

H₂0₂+0-Dianisidine (reduced) Horse Radish O-Dianisidine (Oxidised)+ ₂0

(colourless) > (red colour)

Peroxidase

In all cases the T. flavus (var macrosporus) strains from Dr. J. Pitt gave negative results. The ATCC strains both tested positive for glucose oxidase production. Strain 32908 produced approximately 15 times more glucose oxidase than strain 26015. This correlates well with the inhibition studies where no significant inhibition was seen with those strains not producing glucose oxidase and inhibition levels were much higher with 32908 than 26015. Assays over time also showed glucose oxidase loses approximately half its activity in 3.5 days. Therefore the increased growth in some of the V. dahliae isolates in the later days of the experiment is probably due to inactivation of the glucose oxidase enzyme and a subsequent lowering of H₂0₂ concentration.

Cloning of the glucose oxidase gene from T. flavus.

Because of the high levels of glucose oxidase produced by the ATCC strain 32908 this was obviously the best choice for the cloning of the gene. The A. niger glucose oxidase gene was used as a probe for the isolation of the T. flavus gene as there could be expected to be some homology at the DNA level between the two species. Primers were made to the 5' and 3' ends of the different strands of the A. niger coding region. DNA was isolated from A. niger strain 9029 using the method of Raeer and Broder (1985) and a polymerase chain reaction (PCR) was carried out using 200 ng of this DNA (Cycle = 1 min @ 94°C, 1 min @ 55°C, 3 min @ 72°C - repeated 35X). The expected 1.8 kilobase (kb) fragment was visualised on a gel and restriction enzyme analysis and sequencing confirmed the fragment as the A. niger glucose oxidase gene.

Southern blots of T. flavus DNA were then probed with this fragment to determine if the A. niger gene was sufficiently similar to the T. flavus gene to be used as a probe. Hybridisation was initially carried out at 37°C (with formamide) overnight and the filter washed twice with 1XSSC, 0.1% SDS at room temperature. As seen in Fig. 2, the A. niger gene is clearly visible (16kb) however only a very faint band was seen in the T. flavus lane (2.2kb). Surprisingly A. nidulans which does not produce glucose oxidase also has a faint band present at 3.0kb. The stringency was reduced in an attempt to increase the

T. flavus signal. Hybridisation was carried out at 30°C and the filters washed twice with 2XSSC, 0.1% SDS at room temperature. A band was now clearly visible in the T. flavus lane, this was thought to correspond to the glucose oxidase gene. The A. niger gene was therefore used under these conditions to screen a T. flavus genomic library. A Sau3A genomic library was constructed in ΛEmbl 3 using DNA made from T. flavus 32908. DNA was partially digested with Sau3A, size fractionated on a glycerol gradient and fragments of 18-22kb pooled. SamH1 cut Embl 3 arms were purchased from Promega. DNA was ligated into the arms overnight, packaged and then used to infect E.coli LE392 cells. A total of 50,000 plaques were obtained, 8,000 were screened and four possible positives isolated. Secondary screening revealed two positives, one stronger than the other. Both were purified, liquid lysates prepared and DNA extracted. They were found to contain inserts of approximately 20kb.

DNA from the strongest clone was digested with a number of restriction enzymes, blotted and then probed with the A. niger gene. Only a single band was highlighted in lanes digested with EcoRλ (7.6kb) and Sam -/1 (2.2kb), therefore these fragments were thought to contain the desired glucose oxidase gene. The fragments were cloned into the plasmid pUC119 and mapped. The 7.6kb fragment was found to contain the 2.2kb fragment plus 2.6kb further upstream and 2.8kb further downstream. Specific regions were subcloned into M13 and sequenced.

The sequence of the T. flavus glucose oxidase gene is set out in Table

2. The putative signal sequence is underlined. Possible TATAA and CAAT boxes are double underlined. Translation of the entire sequence is shown beginning at the ATG start site, (nucleotide #1).

TABLE 2 Sequence of T. flavus glucose oxidase gene (SEQ.ID NO:1)

-1032

CCACAAGTCCTAGAGAAGACACACAGTCTCGAGCCCAAAGTAAGAATGGATATTGTGACT

-972

TCCTAAAGGCCTCACCGGGCAGTGAGGTATTTGATGTTTACCAAACGCTAGTATGGGTAG

-912

CATAATCGGTGATACCTAGGTATATCATATGTTCATCCACAGGGCTGGGTTTGTGAAGAA

-852

ACTGTAGCACTAGTGCTGCTTAGTTGCATATGGAGTTTCTATCTGCACTATTCCGTTGGA

-792

GGAAGGAAGAAAAGGGCAAGAGAGATACTGTCAAATGAATGTACTCGGGGGTCACTGAAT

-732

ACGTGAAAGCGTACTTAGGTGATCTATTGCGAGAATAGTTCAATGATATCGATGTCCTCT

-672

CGGCGCTCCACTCTCTCTATTCGTATCTGATTCTGATCTGCTCTTCATTCACAACTTTAT

-612

GTATCTGTCATGCCAGTTTTACGAGTACTGGGAAAGTTGGCGCTCAGAGCTGGGATTCTT

-552

GGGTTTCATTGACGCTCAACCTAGAGTTTGAATGATATCGCTTTATCTTTAGATAATCTT

-492

CAACGTAACAATGTGCTTGAGCTTCTAGCGCCAAGATGCGTAGACTTTCGTAAATGGTAG

-432

TTCAAGCTAATAATTCAGGAAAATATTGCAGAGGATTATCGCCACACATGCCGATGGAGC

-372

ATACAGACTCCTCTTGATACGATGCTTTGACCACTCACATCCTCCAGCCTTCCATCCAGG

-312

TCCCTAGGTTCAGCCGTGCTTCCAGCACTTACTGATCAAACCCCTGTAGCACGGCTAGTA

-252

TCTCATATCTTTCCGTCTGCAGCATGAGTCGCTCATGTCTGCACGAGTCCATTTTCAGAA

-192

AGTGGGATAATCTAACCTGGTGGCGAGGCCAAGATACGACATAAAGGAAATGTTTGCTTC

-132

TTGCAAGTCTATAAATTGAGCGACATCTACCGCTGTTCAGACAAGTTCTTCAGCACAACA

-72

ATCAGGTAATTTCACCACTCTCCTTGCAATCCCGTTTATCTTCTCCATCTCCTTGACCTT

-12

M V S V F L S T L L L A A A T V GCCGGATCGAAATGGTGTCTGTATTTCTCAGCACTCTTCTTTTAGCCGCGGCTACGGTC 47

Q A Y L P A Q Q I D V Q S S L L S D P S CAAGCCTACCTGCCTGCCCAACAGATTGATGTCCAGTCTAGTCTTCTCAGTGACCCTAGC 107

K V A G K T Y D Y I I A G G G L T G T AAGGTCGCCGGAAAGACCTATGATTACATTATTGCTGGTGGTGGTTTGACTGGCCTTACT 167

V A A K L T E N P K I K V L V I E K G F GTTGCCGCCAAACTGACAGAAAACCCCAAGATCAAAGTCCTGGTTATTGAAAAGGGCTTC 227

Y E S N D G A I I E D P N A Y G Q I F G TATGAGTCCAACGATGGAGCCATCATCGAGGATCCAAATGCTTACGGACAAATCTTCGGC 287

T T V D Q N Y L T V P L I N N R T N N I ACCACTGTTGACCAGAACTACCTCACCGTTCCCCTGATCAACAACCGCACGAACAATATC

347 K A G K G L G G S T L I N G D S W T R P AAGGCCGGCAAGGGTCTTGGAGGATCAACCTTGATAAACGGTGACTCTTGGACTCGCCCG 407

D K V Q I D S W E K V F G M E G W N W D GACAAAGTCCAGATTGATTCTTGGGAGAAGGTCTTTGGCATGGAAGGTTGGAATTGGGAC 467

S M F E Y M K K A E A A R A P T A A Q L AGTATGTTTGAGTACATGAAGAAGGCCGAGGCTGCACGTGCCCCTACTGCTGCTCAACTT 527

A A G H Y F N A T C H G T N G T V Q S G GCTGCCGGTCACTACTTCAATGCTACCTGCCATGGAACTAACGGTACTGTTCAATCCGGA 587

A R D N G Q P S P I M K A L M N T V S GCCCGTGACAACGGTCAACCTTGGTCTCCTATTATGAAGGCCCTTATGAACACCGTCTCG 647

A L G V P V Q Q D F L C G H P R G V S M GCCCTTGGTGTCCCCGTACAGCAAGACTTTCTCTGCGGTCATCCTCGAGGTGTCTCTATG 707

I M N N V D E N Q V R V D A A R A L L ATCATGAACAATGTCGACGAAAACCAAGTTCGTGTTGATGCTGCCCGTGCATGGCTGCTT 767

P S Y Q R P N L E I L T G Q M V G K V L CCCAGCTACCAGCGCCCCAACTTGGAGATCCTTACTGGTCAGATGGTTGGAAAGGTTCTG 827

F K Q T A S G P Q A V G V N F G T N K A TTTAAACAGACCGCATCCGGTCCCCAGGCTGTTGGTGTGAACTTCGGTACTAATAAGGCC 887

V N F D V F A K H E V L L A A G S A I S GTTAACTTTGACGTCTTTGCTAAGCATGAGGTCCTTTTGGCTGCCGGCTCAGCTATCTCT 947

P L I L E Y S G I G L K S V L D Q A N V CCGCTGATCTTGGAATATTCTGGCATAGGCTTGAAGTCTGTTCTTGATCAGGCCAATGTC 1007

T Q L L D L P V G I N M Q D Q T T T T V ACTCAGCTTCTTGATCTTCCTGTTGGTATCAATATGCAAGACCAGACCACAACCACTGTC 1067

S S R A S A A G A G Q G Q A V F F A N F AGTTCCCGTGCTAGTGCCGCTGGTGCTGGTCAGGGTCAGGCCGTCTTCTTCGCCAATTTC 1127

T E T F G D Y A P Q A R E L L N T K L D ACTGAAACCTTCGGTGACTACGCCCCCCAGGCCAGAGAGTTACTCAACACCAAGCTTGAC 1187

Q W A E E T V A R G G F H N V T A L K V CAATGGGCTGAGGAGACCGTTGCGCGAGGTGGTTTCCATAATGTAACTGCTCTCAAAGTT 1247

Q Y E N Y R N L L D E D V A F A E L F CAATATGAAAACTATCGTAACTGGCTCCTTGACGAAGACGTTGCCTTCGCCGAGCTTTTC 1307

M D T E G K I N F D L D L I P F T R G ATGGATACCGAGGGCAAGATCAACTTCGACTTATGGGATCTCATCCCTTTCACTCGTGGT

1367

S V H I L S S D P Y L Q F A N D P K F TCCGTCCATATCCTCAGTAGCGACCCTTACCTATGGCAATTCGCCAACGACCCCAAATTC 1427

F L N E F D L L G Q A A A S K L A R D L TTCCTGAACGAGTTTGACCTCCTTGGTCAAGCCGCTGCTTCCAAGCTTGCTCGTGATCTT 1487

T S Q G A M K E Y F A G E T L P G Y N L ACCAGCCAAGGTGCTATGAAGGAGTACTTCGCCGGAGAGACTCTTCCAGGATACAACTTG 1547

V E N A T L S Q W S D Y V L Q N F R P N GTCGAGAATGCTACTCTTTCCCAGTGGTCGGATTATGTCTTACAGAACTTCCGTCCCAAC 1607

W H A V S S C S M M S R E L G G V V D A TGGCATGCTGTCAGCAGCTGCTCTATGATGTCTAGAGAGCTTGGTGGTGTCGTTGATGCT 1667

T A K V Y G T Q G L R V I D G S I P P T ACTGCCAAGGTGTACGGTACGCAGGGCCTACGTGTCATTGATGGCTCTATTCCTCCGACT 1727

Q V S S H V M T I F Y G M A L K V A D A CAGGTGTCTTCTCATGTCATGACCATTTTCTACGGAATGGCTTTGAAAGTTGCTGATGCG 1787

I L D D Y A K S A * ATTCTGGACGACTATGCCAAAAGTGCCTAGAGGTGTCATGAATCGCGGTTCGTCAGCGAA 1847

TTTGCTAGGGTTTAGATCACCGATTTTTTCTCCTCGCTCATACATTGTTAGATTCTCGCA 1907

CATATAGATCGATTTAAATTGCTTATAGACAACGTGAAATTTACTACTTATTCATCGAAC 1967 TTACATTCTTCAAAATATTCAAGAGAGCTC

Approximately 3.0kb of T. flavus DNA has been sequenced on both strands. Analysis has revealed a 1815bp open reading frame (ORF) from bas 1032 to base 2847, (Table 2). This ORF is exactly the same size as the A. niger glucose oxidase open reading frame and is 65% homologous to it at a nucleotide level. Comparisons show that the T. flavus gene has undergone an insertion at bases 1089 to 1091 of a leucine amino acid and a deletion at bases 1349 to 1351 of a glutamic acid residue. At an amino acid level the T. flavus gene is 64% homologous to the A. niger glucose oxidase protein (77% similarity). Hydrophobicity plots of the two proteins show them to be very similar. Like the A. niger ORF, T. flavus contains a putative secretion signal sequence at the beginning of the ORF. This sequence seems to extend for approximately 20 amino acids and consists predominantly of hydrophobic amino acids. All this strongly suggests that ORF corresponds to the coding region of the T. flavus glucose oxidase gene.

As no conserved regions have been clearly defined for fungal untranslated flanking regions it is difficult at this stage to define essential sequences in these regions. There is a possible TATAA sequence at -122, and two CAAT boxes are present at -43 and -73 (wrt to the ATG initiation codon). The CAAT boxes are within a very pyrimidine rich region (74%) which spans from -12 to -73 bases upstream. Such regions have been found in many fungal promoters and may be important in positioning the site of transcription initiation (Hammer and Timberlake, 1987). No AATAAA polyadenylation sequence has been found. This 3' region is however quite AT rich, 64%. This compares with 50% for the coding region and 55% for the 5' untranslated region.

Demonstration of Glucose Oxidase activity on the cloned DNA sequence.

As all of the macrosporus biotypes of the T. flavus were not producing glucose oxidase these were useful recipients to demonstrate that the cloned gene was indeed functional. A transformation procedure for T. flavus had to be developed to allow the introduction of the glucose oxidase gene into one of these strains. Such transformants could also be tested for their antagonistic properties towards V. dahliae to further characterise the role glucose oxidase in the mycoparasite relationship between these organisms. Additionally, some of the transformants may be better glucose oxidase producers than 32908 and could be useful as biocontrol agents (strain 32908 may not be able to be used in the field because of quarantine regulations).

Many different filamentous fungi have now been transformed although the frequencies reported are often very low when the protoplast method is used. In this method the cell wall is digested away in the presence of an osmotic stabiliser to produce spheroplasts. These are exposed to DNA in the presence of CaCI₂ and polyethylene glycol (PEG) which promote DNA uptake. Following treatment, the spheroplasts are allowed to regenerate in an osmotically stabilised medium at which time selective pressure is applied. The basic procedure followed is that of Murray et al., 1992. The recipient strain used was FRR 2417 as this had been obtained from Australian soil. Preliminary experiments showed this strain to be sensitive to moderate concentrations of hygromycin, (200 μg/ml) so initial transformations were done with the vector pAN7-1 (Punt et al., 1987) which carries the gene for hygromycin resistance under the control if A nidulans 5' and 3' sequences. Before transformation the vector was linearised with Hind\\\ as linear DNA is thought to be more recombinogenic than circular DNA (Orr-Weaver et al., 1981).

Hygromycin resistant colonies were observed 1-2 weeks after transformation. Approximately 20 transformants///g of DNA were obtained. This corresponds to a transformation frequency of about 0.001% of the original number of protoplasts or 0.01-0.02% if one takes into account that only 5-10% of the protoplasts regenerate after incubation in PEG. Southern blotting and probing of transformant DNA with pAN7-1 confirmed the presence of the hygromycin gene in the fungal genome. Size and number of fragments hybridizing differs from transformant to transformant. As DNA was cut with EcoRV, an enzyme which does not cut within the vector, hybridizing fragments represent one copy or several tandem repeats of the vector. Differences in fragment size are therefore caused by integration of the vector into different places in the fungal genome. Multiple fragments arise when the vector integrates into a number of different sites in the transformant genome.

The 7.6kb EcoR1 fragment believed to contain the T. flavus glucose oxidase gene was cotransformed into FR 2417 with pAN7-1. Transformants were initially selected on hygromycin and then these colonies screened on both indicator plates. A similar transformation frequency was obtained, (0.01%). Of 29 transformants analysed, 18 were glucose oxidase positive and 11 negative, i.e. a cotransformation frequency of 62% and clearly demonstrated that the 7.6kb EcoR fragment contained a functional T. flavus glucose oxidase gene.

Glucose oxidase expressed in a non-producing strain is toxic to Verticillium. Talaromyces flavus var macrosporus is a non-glucose oxidase producing strain that has no antagonistic activity against fungi such as Verticillium. Transgenic macrosporus strains expressing the cloned glucose oxidase gene were tested for antifungal effects using culture filtrates as described in Figure 1. The transformed fungi produced copious amounts of glucose oxidase and this proved toxic to Verticillium (Figure 1), although the growth suppression was not quite as large as for the native glucose oxidase producing strain, perhaps indicating that there may be some other components to the growth inhibition. This strain has yet to be tested for biocontrol properties in vivo.

EXAMPLE 2

Glucose Oxidase is toxic to insect larvae.

H. armigera larvae can be reared on a synthetic medium containing soybean flour, wheat germ, yeast and various vitamins and oils. When glucose oxidase (from Aspergillus niger, Sigma Co.) was incorporated into the diet at 1 mg/ml it did not affect larval growth or survival except when glucose (8% w/v) was also present (Table 3) when assessed after 7 days.

TABLE 3 Effect of glucose oxidase on larval survival and growth.

Treatment Survivors Average Wt Wt% of (mg) Control

Control (added water) 10/12 10.5 100

Control + Glucose oxidase 11/12 8.4 80

Control + Glucose oxidase + Glucose 0/12 0 0

Control + Glucose 9/12 2.8 27

Control + Sucrose 9/12 2.6 25

Control + Sucrose + Invertase 12/12 2.5 24

Control + Sucrose+lnvertase+Glucose Oxidase 7/12 0.7 6.6

No survivors were present in the glucose oxidase plus glucose treatment whereas all other treatment had significant numbers of survivors out of the 12 larvae tested. Surprisingly some of the control treatments with sugars had some effects on growth rates perhaps because of greater bacterial or fungal growth in the medium. Glucose generated by the action of yeast invertase (1 mg/ml) on sucrose could partially substitute for glucose added to the medium although this was not sufficient to kill all of the insects. Similar results were obtained on two separate occasions.

EXAMPLE 3

Expression of T. flavus glucose oxidase in transgenic plants.

MATERIALS AND METHODS

Gene constructions.

Glucose oxidase plasmids All DNA manipulations were performed using standard procedures (Sambrook et al., 1989). A 2.2kb Pst/Sac\ fragment containing the T. flavus glucose oxidase open reading frame in addition to approximately 250 bp of 5' and 150bp of 3' DNA was subcloned into pBluescript SK~(Stratagene) to create pGO. The 4kb EcoRI DNA fragment from PDC5A1 was recloned into the EcoRI restriction site of pJKKm creating pDC5A2. Restriction mapping revealed a Kpn\ site approximately 3kb downstream from the 5' EcoRI site of the extensin fragment. This 3kb Kpn\ fragment from PDC5A2, was subcloned into pBluescript SK^" to create pEx. In vitro mutagenesis was carried out with either pG01 or pEx to introduce restriction enzyme recognition sites around the ATG and 3' end of the putative secretion signal peptides of both genes. The presence of the correct mutations was confirmed by restriction digest analysis. The following synthetic oligonucleotides were used: G01 CCTTGCCGACTAGTAATGGTGT (SEQ ID NO:2) G02 CCTACCTGGATATCCAACAGAT (SEQ ID NO:3)

Ex1 TTGGTTGTACTAGTCATGGGAA (SEQ ID NO:4)

Ex2 CCACAGCTGTTAACACTTACTC (SEQ ID NO:5)

The following plasmids were created, pGO-1, which had a Spel site introduced just prior to the initiating ATG of the T. flavus glucose oxidase gene; pGO-2, which had an EcoRV site introduced at the 3' end of the putative 7. flavus glucose oxidase signal peptide; pEx-1, which has a Spel site introduced just prior to the initiating ATG of the carrot extensin gene; pEX-2, which has a Hpal site introduced at the 3' end of the putative carrot root extensin signal peptide and a Spel site introduced just prior to the initiating ATG of the extensin gene.

Plasmid pFGOEN

The Spel/Sacl DNA fragment from pGO-1 containing the glucose oxidase gene and 5' signal peptide was subcloned into pBluescript SK- to create pGO-

1A. The Spel/EcoRI fragment from pEx-1 was cloned into the Spel/EcoRI restriction sites upstream of the glucose oxidase gene in pGO-1A to create pFGOE. The EcoRI/Sacl fragment from pFGOE containing the glucose oxidase gene and signal peptide fused to the extensin promoter was then subcloned into the EcoRI/Sacl restriction sites of pGN 100 (Bogusz et al., 1990) to create PFGOEN-1.

Plasmid pEGOEN

The 2.2 kb Pst\/Sac\ fragment from pG02 containing the glucose oxidase gene into which Hpal restriction site had been engineered, was subcloned into the pstt/Sac\ restriction sites in pJKKm (Kirschman and Cramer, 1988). This plasmid was digested with EcoRV/EcoRI and the 1.9kb fragment containing the glucose oxidase gene cloned into pBluescript SK^" to create pG02A. To create PEGOE, the 0.75kb Hpa\/Kpn\ DNA fragment from pEx-2 containing the extensin promoter and secretion signal peptide was subcloned into the EcoRV/EcoRI restriction sites upstream of the glucose oxidase gene in pG02A. The EcoRI/Sacl fragment from pEGOE containing the extensin promoter, signal peptide and glucose oxidase gene was then subcloned into the EcoRI/Sacl restriction sites of pGN100 to create pEGOEN.

Plasmid pFGOTN The TobRB7 promoter was subcloned into pBluescript SK^" to create pTobRB7-2. To create pFGOTN, the extensin promoter in pFGOEN was relaced with the pTobRB7 promoter by cloning the Spel/EcoRI fragment from pTobRB7-2 into the Spel/EcoRI restriction sites of pFGOEN.

Plasmid pEGOTN

The plasmid was created by replacing the Spel/EcoRI extensin promoter fragment from pEGOEN with the Spel/EcoRI TobRB7 promoter fragment from pTobRB7-2.

Plasmid pFGOSN

The Pst\/BamH\ DNA fragment from 35SKNΔBam (J. Walker, unpublished) containing the 35S promoter was sucloned into the Psfl/SamHI restriction sites in pBluescript SK^" to create p35S-1. Plasmid pFGOSN was created by replacing the Spel/EcoRI extensin promoter fragment in pFGOEN with the Spel/EcoRI DNA fragment from p35S-1.

Plasmid pEGOSN

The EcoRI/Spel fragment from pEGOEN containing the extensin promoter was replaced with the EcoRI/Spel fragment from p35S containing the 35S promoter.

Gene fusions occurring within an open reading frame were checked by dideoxy sequencing using a Pharmacia T7 sequencing kit to ensure the correct open reading frame was conserved. All of the above plasmids were linearized with EcoRI and cointegrated into the binary vector pTAB5 in the opposite orientation to the selectable kanamycin gene. Triparental mating was employed to transfer the binary vector constructs to the super-virulent disarmed Agrobacterium tumefaciens strain AGL1 (Lazo et al., 1991) and constructions were verified by restriction enzyme analysis.

Plant transformations. Transformation of N. tabacum (Wisconsin 38) using A. tumefaciens was performed as described in Lyons et al., (1989). Plants were subcultered every 6-8 weeks to fresh MS medium containing 3% sucrose and 0.8% agar. Seed from Gossypium hirsutum (cv Coker 315) were surface sterilized and transformed as described in Cousins et al (1991) with the following modifications. After 2 days co-cultivation with the appropriate A. tumefaciens strain each explant was transferred to callus initiation media containing 50 mg/l kanamycin. Six weeks later callus was subcultered to the same media containing 25 mg/l kanamycin. After a further six weeks surviving callus was subcultered to solidified basal medium containing no hormones or antibiotics. Embryos formed 5-12 weeks later, large embryos forming roots were transferred to deep petri dishes containing Stewart and Hsu (1977) medium solidified with Phytogel and magnesium chloride. Analysis of plant tissue for the presence of glucose oxidase.

Glucose oxidase activity was assayed qualitatively by submerging small pieces of plant tissue in Kl/starch stain. Tissue was incubated overnight at room temperature before being scored for activity. For quantitative glucose oxidase assays, leaf or root tissue removed from plants propagated in tissue culture, was homogenized with 0.1M Na₂P0₄ buffer (pH 6.0) in a mortar and pestle. Homogenate was poured into eppendorf tubes and centrifuged at 13000rpm for 15 minutes. The supernatant was removed and incubated at 4°C for 2-3 hours before it was assayed for the glucose oxidase activity. Protein concentration was determined by the method of Bradford (1976) and measured using a Labsystems Multiskan Plus.

PCR reactions.

Isolation of Genomic DNA Genomic DNA was isolated from young leaves of tobacco plants propagated in tissue culture. One leaf was homogenized in an eppendorf tube containing 300/ I of grinding solution (comprised of 1.25ml of TE3D buffer, (0.02M Tris, 002M Na₂EDTA, 1% Nonadet P-40, 1.5% lithium dodececyl sulphate and 1% sodium deoxycholate) 2.5ml of equilibritated phenol and 50//I of /?-mercaptoethanol). After homogenization, 250/ I of ammonium acetate/EDTA solution (3M ammonium acetate, 0.4mM Na₂EDTA, 0.18M NaOH) and 400//I of chloroform was added and the tube mixed for 20 minutes. The tube was centrifuges at 13000rpm at 4°C for 10 minutes, the supernatant removed and DNA precipitated by the addition of 0.6 volumes of isopropanol. The pellet was resuspended in TE buffer and treated with Ribonuclease A (previously boiled) then extracted with phenol/chloroform, ethanol precipitated and resuspended in distilled water.

PCR conditions The following oligonucleotide primers which are complementary to two regions in the T. flavus glucose oxidase open reading frame (position 681 and 1513 with respect to the initiating ATG) were synthesized on an Applied Biosystems DNA synthesizer.

FMG03A 5' GCGGTCATCCTCGAGGTGTCTCTATG 3' (SEQ. ID NO:6) GOFM4 5' TACTCCTTCATAGCACCTTGGCTGGT 3' (SEQ. ID No:7) PCR was carried out using either 250ng of tobacco genomic DNA or 40 ng of pEGOSN plasmid DNA and Taq DNA polymerase buffer (Promega); 2.5mM MgCI₂; 200 /M each dNTP; 1 /M each primer and 2.5 units of Taq DNA polymerase (Promega). The reaction consisted of 30 cycles: cycle 1 = 5 min @ 94°C, 2min @ 55°C, 2 min @ 72°C (performed once) cycle 2 •= 1 min @ 94°C, 1min @ 55°C, 2min @ 72°C (performed 29 times) cycle 30 = 5 min @ 30°C (performed once)

PCR reaction products were visualized by running the completed reaction on a 0.7% agarose gel.

Northern analysis.

Total RNA was extracted from young tobacco leaves excised from plants being propagated in tissue culture using the method of Dolferus et al (1994). Equal amounts (20//g) of total RNA was loaded on 1.1% agarose gels containing 2.2M formaldehyde in the presence of ethidium bromide. After electrophoresis the gels were transferred and UV cross-linked onto Hybond-N nylon membranes (Amersham). The plasmid pGO-1A which contained the entire T. flavus glucose oxidase open reading frame was used to generate a riboprobe to detect glucose oxidase RNA. This plasmid was linearized with EcoRI and an antisense [³²P]UTP-labelled riboprobe was made using T3 polymerase and a Promega in vitro transcription kit. An antisense riboprobe corresponding to an Arabdopsis ubiquitin clone (Burke et al., 1988) was used to quantitate the amount of tobacco RNA. RNA probe hybridizations and washing of filters was carried out as described in Dolferus et al (1994). Filters were exposed to X-ray film at ^"80°C for 2-3 days. Analysis and quantitation of the hybridization signals was performed with a phosphorimager (Molecular Dynamics, Sunnyvale, CA). RESULTS

Construction of plasmids for the expression of T. flavus glucose oxidase in plants. As the glucose oxidase gene isolated was of fungal origin, it was not known if the secretion signal peptide at the 5' end of the gene would function correctly in plants. To obtain good gene expression, the presence of a functional signal peptide was thought to be important for two reasons. First, glucose oxidase is glycosylated protein, lack of glycosylation caused by a nonfunctional signal peptide could decrease enzyme activity. Secondly, because of the potential toxicity of the hydrogen peroxide produced by glucose oxidase, it would be desirable to have the enzyme excreted from the cell. The effect replacing the fungal signal peptide with one from plants has on glucose oxidase gene activity is not known. Such a substitution could decrease gene expression and or protein activity. To avoid these potential problems, two different series of expression vectors were made. In the pFGO series, the glucose oxidase secretion signal peptide was retained. In the pEGO series, the final signal peptide was replaced with the secretion signal peptide from the carrot extensin gene (Chen and Varner, 1985) as described in Material and Methods. This plant signal peptide was used, as a similar extensin signal peptide from tobacco has been shown to mediate the secretion of neomycin phosphotransferase II (npfll) from tobacco protoplasts (Loose et al., 1991).

in order to successfully express the glucose oxidase gene plants, root specific or inducible gene expression may be necessary because of the potential toxicity of the hydrogen peroxide to the plant. The glucose oxidase gene and signal peptide from each of these plasmids was therefore joined to three different promoters as described in Materials and Methods. The promoters used were the 35S promoter from cauliflower mosaic virus, the TobRB7 promoter from tobacco (Yamamoto et al., 1991) and the extensin carrot root promoter (Chen and Varner, 1985). Each of these promoters directs a different pattern of gene expression in plants. The 35S promoter constitutively expresses genes in most plant tissues (Odell et al., 1985), TobRB7 directs constitutive, root specific gene expression (Yamamoto et al., 1991) and the extensin carrot root promoter has been shown to be wound inducible in carrot roots (Chen and Varner, 1985).

As described in Materials and Methods, each construct was fused to a

NOS 3^' terminator and then cloned into the EcoRI site of the binary vector pTAB5 (Tabe et al., 1995). Restriction enzyme analysis was performed on all constructs to confirm the correct integration and orientation of the glucose oxidase gene in the binary vector (results not shown). Constructs containing the glucose oxidase gene in an indirect orientation to that of the 35S-npfll gene (kanamycin resistance) were introduced into tobacco by way of Agrobacterium- mediated transformation. Diagrams of the plasmids, pEGOE (carrot root extensin promoter), pEGOT (pTobRB7 promoter) and pEGOS (35S promoter) are shown in Figure 3. These constructs all contain the extensin secretion signal peptide. The three constructs containing the glucose oxidase secretion signal peptide attached to the glucose oxidase gene (pFGO series) are also shown and are identical to the pEGO series except that they have the glucose oxidase secretion signal peptide instead of the extensin secretion signal peptide.

Expression of T. flavus glucose oxidase in Nicotiana tabacum.

For each of the six constructs, fifteen to twenty transgenic tobacco plants were regenerated. Glucose oxidase activity in transgenic plants was assayed qualitatively by submerging small pieces of plant tissue into a solution of glucose, potassium iodide, (Kl) and soluble starch. In transgenic plants expressing functional glucose oxidase, hydrogen peroxide produced by glucose oxidase, oxidises the Kl to iodine (l₂). The l₂ then interacts with the starch to form a blue-black starch complex. The presence of glucose in the strains solution was not necessary for the formation of the blue-black colour but its presence did greatly increase speed of colour formation. A similar solution has been used by Olson and Varner (1993) and Schopfer (1994) to detect endogenous hydrogen peroxide in plant tissue. However, when tissue is completely submerged in stain solution (anaerobic conditions) no endogenous activity is detected. This stain solution can therefore be used under these conditions to assay for glucose oxidase activity.

As seen in Table 4, glucose oxidase activity could be detected in only three of the sixty tobacco plants obtained from transformation with constructs in which the glucose oxidase gene retained its own secretion signal peptide (pFGO series). Very weak staining was observed in all three transformants so the glucose oxidase activity in these transformants is thought to be very low. Many of the plants (58%) obtained from transformation with constructs containing the glucose oxidase gene attached to the extensin secretion signal peptide (pEGO series) did show glucose oxidase activity. In particular, 80% of the plants transformed with constructs in which the glucose oxidase gene was driven by the 35S and TobRB7 promoter showed activity.

Table 4 Glucose oxidase activity in transgenic tobacco transformed with different constructs. All plants are believed to be independent transformants. Activity was determined qualitatively using a Kl/starch solution. Each plant was tested three times, the results were identical each time.

Construct used to Number of positive transform W38 transgenic plants

Tobacco in Kl stain pEGOS 13/15 pEGOT 11/15 pEGOE 2/15 pFGOS 3/20 pFGOT 0/20 pFGOE 0/20

Untransformed W38 0/5

Analysis of glucose oxidase expression in T1 progeny.

To obtain plants for further analysis, plants expressing the glucose oxidase gene controlled by the 35S and TobRB7 promoter (pEGOS and pEGOT constructs) were potted in soil and transferred to the glasshouse where they were propagated further. In soil, all plants appeared to grow normally and all plants produced flowers and pollen. Seeds were obtained from all plants containing plasmid pEGOT. Only six of the ten plants containing the glucose oxidase gene controlled by the 35S promoter (pEGOS) produced seed. Compared to W38 untransformed plants, four of these six plants, had small seed pods which contained few seeds. The other two plants produced seed pods containing a similar number of seeds and of similar size to seed pods produced by untransformed W38 tobacco plants.

Seeds from eleven of the transgenic plants were surface sterilized and germinated on agar medium. To detect glucose oxidase activity, seedlings from each plant were stained with Kl solution. Some localization of gene expression was seen, staining occurs over the entire seedling in seedlings containing pEGOS but is confined to the root in seedlings containing pEGOT.

Thirty seedlings from each plant were randomly chosen and scored for glucose oxidase activity by staining with Kl/starch solution (Table 5). It was not possible however, to determine whether seedlings were homozygous or hemizygous for the glucose oxidase gene using this method. Except for seedlings from plant GOS-13, glucose oxidase activity was detected in approximately 75% of the seedlings from each plant (Table 5). Approximately 96% (29/30) of the seedlings from GOS-13 tested displayed glucose oxidase activity. Seeds were also germinated one medium containing kanamycin and scored for survival (Table 5). Three percent of GOS-13 seedlings and approximately 25% of the other seedlings tested germinated bleached and later died. Therefore, in most plants the glucose oxidase and kanamycin resistance gene segregates in a Mendilian 3:1 ratio. The higher frequency of the glucose oxidase and kanamycin resistance gene in GOS-13 progeny could result if the T-DNA has integrated into two different loci. In this situation only 1/16 seedlings (approximately 6%) would be expected to not have glucose oxidase activity. The occurrence of two different integration events could also result in the high level of glucose oxidase activity found in GOS-13. Table 5 Inheritance of the glucose oxidase and kanamycin resistance gene in T1 transgenic tobacco seeds, a: Seedlings were stained with

Kl/starch solution to determine glucose oxidase activity, b:

Seedlings were germinated on media containing 100 //g/ml kanamycin to determine presence of npfll gene.

Plant Percentage of T1 seedlings Percentage of surviving T1 producing glucose oxidase.⁸ seedlings." (of 30 scored)

(of 30 scored)

EGOS-9 77 73

EGOS-13 97 97

EGOS-24 73 83

EGOT-2 80 83

EGOT-9 73 70

EGOT-10 67 77

EGOT-15 67 83

EGOT-17 83 70

EGOT-18 67 73

EGOT-19 80 70

EGOT-21 73 83

Expression of glucose oxidase in Gossipium hirsutum.

Plasmids pEGOT (Glucose oxidase gene driven by the TobRB7 promoter and extensin signal peptide) and pEGOE (glucose oxidase gene driven by the extensin promoter and extensin signal peptide) were separately transformed into G. hirsutum cv. Coker by way of Agrobacterium mediated transformation. Calli was selected from each of the transformations on kanamycin containing medium and regenerated into plants as described in Materials and Methods.

Approximately 50% of the callus derived from tissue transformed with pEGOE died 3-4 months after the transformation however 16 plants from independent transformation events were still regenerated. 34 plants from independent transformation events were regenerated after transformation of cotton with pEGOT. Roots from at least three clones of each line were tested for glucose oxidase activity in Kl/starch stain solution before being transferred to the pots in the glasshouse. Three of the 16 lines regenerated after transformation with pEGOE and 23 of the 34 lines generated after transformation with pEGOT produced glucose oxidase (Table 6).

Plants were placed into different groups depending on the time taken for the Kl/starch stain solution to completely change colour after the addition of roots to the solution. Group 1 roots completely changed the colour of the stain solution within one hour of being added to the solution, Group 2 within four hours, Group 3 overnight and Group 4 never completely changed the colour of the solution but some staining of solution and roots was observed (Table 6). Glucose oxidase activity ranging from weak to strong is seen in cotton plants transformed with pEGOT. Only very weak activity is seen in cotton plants transformed with pEGOE.

All sixteen cotton lines regenerated after transformation of cotton with pEGOE and the 23 lines regenerated after transformation with pEGOT which are expressing glucose oxidase are being progated further in the glasshouse. To date, six lines containing pEGOT have flowered, self pollinated and set seed

(Table 6).

TABLE 6 Regenerated cotton lines producing glucose oxidase. Each line is believed to represent an independent rransformatikon event. Cotton lines were placed into different groups based upon the time taken for three 2cm roots to completely change the colour of 250 μ\ of Kl/ starch solution.

Regenerated cotton lines Total number of producing glucose oxidase. plants in group.

Plants containing pEGOT

Group 1 T-53, T-76*. T-78, T-97 4

Group 2 T-2*, T-10, T-12, T-13, T-24*. T- 11 52, T-71, T-77, T-90, T-92*. T-105

Group 3 T-5, T11, T-14*, T-16. T-68* 5

Group 4 T-48*. T-99, T-19 3

Plants containing pEGOE

Group 1 0

Group 2 - 0

Group 3 - 0

Group 4 E-42, E-60, E-91 3

Indicates those lines which have flowered and formed bolls.

EXAMPLE 4

Resistance of transgenic tobacco plants expressing glucose oxidase to Rhyzoctonia solani.

Australian isolates of V. dahliae do not infect tobacco so the glucose oxidase producing transgenic tobacco plants described in Example 3 could not be tested for increased resistance to verticillium wilt. Another soil borne fungus, Rhyzoctonia solani has been found to be susceptible to low concentrations of hydrogen peroxide by Kim et al., 1990^a". This fungus infects many different plant species including tobacco and usually invades the hypercotyl of young seedlings where it decays stem tissue eventually causing the seedling to collapse. The pathogen is not a major problem in agriculture as it is readily controlled by fungicides or as cool, wet conditions early in growing seasons have been found to favour disease development, losses can be greatly reduced by delayed planting.

An Australian isolate of R. solani originally isolated from cotton was found to infect W38 tobacco under favourable conditions, and this isolate has been tested for its tolerance to glucose oxidase and found to be moderately sensitive to the enzyme. To determine if plants expressing glucose oxidase are resistant to R. solani infection, T1 tobacco seedlings expressing the T. flavus glucose oxidase gene under control of either the 35S or TobRB7 promoter are tested for increased ability to survive in sand infested with the R. solani isolate.

MATERIALS AND METHODS

Fungal Isolates.

A R. solani isolate previously isolated from cotton was kindly supplied by Dr. Michael Priest, NSW Department of Agriculture, Rydalmere, Australia. The T. flavus and V. dahliae strains used are described above.

R. solani infection trials.

Tobacco seeds (Wisconsin 38 and transgenic derivatives) were surface sterilised by placing seeds in 70% ethanol for 1 minute and then transferring to a 10% bleach solution containing 1 drop/100 ml of Tween 20 for 10 minutes. After washing five times with sterile distilled water, seeds were placed on MS media containing 100 / g/ml kanamycin and germinated in the light at 26°C. R. solani was grown at 26°C on potato dextrose agar for 7 days. Mycelium was removed from plates with a spatula and blended with sterile nutrient solution (Hoagland No.2 solution (Hewitt, 1966) and 0.5% glucose) for 30 seconds in a Waring blender. Mycelial fragments were filtered through 2 mm nylon mesh before being counted with a "Weber Scientific" counting chamber. Sand (300 ml) was previously dispensed into containers (13cm x 11cm) and autoclaved twice. R. solani mycelial fragments were mixed with nutrient solution and the solution poured evenly over sand in the containers (4x10⁸ mycelial fragments/container). 21 -day-old tobacco seedlings were removed from agar and planted directly into the sand. Containers were covered with clingwrap and placed in an "Environ Air" growth cabinet for 5-6 weeks (24°C, 12 hours light; 20°C, 12 hours dark). Seedlings were removed from sand, washed in water and blotted dry on blotting paper. After weighing, a small mount of tissue was placed in Kl/starch stain to test for glucose oxidase production.

RESULTS

Effect of glucose oxidase on the growth of Rhyzoctonia solani.

Glucose oxidase was examined in vitro for its ability to inhibit the growth of an Australian isolate of R. solani. Different concentrations of A niger glucose oxidase suspended in potato dextrose broth and different amounts of filtrate from T. flavus 32908 and GOH-1 were inoculated with R. solani and fungal growth was monitored using a microtitre plate reader. Duplicates were performed for each experiment and the experiment was repeated twice.

As shown in Figure 4, filtrate from T. flavus 32908 broth and broth containing A. niger glucose oxidase were found to significantly inhibit R. solani growth. The growth profile of R. solani in PD broth alone, PD broth plus gluconic acid or in filtrate from GOH-1 was very similar indicating that as in V. dahliae, it is the hydrogen peroxide produced by glucose oxidase which is toxic to R. solani. Growth inhibition curves for R. solani were calculated 26 hours after the start of fungal growth (Figure 5). Approximately 4.4 /g/ml of A. niger glucose oxidase and the equivalent of 4.1 //g/ml of glucose oxidase in T. flavus 32908 filtrate was required to inhibit R. solani growth by 50% (IC₅₀). These values are approximately twice the glucose oxidase IC₅₀ value determined for V. dahliae (2.2 //g/ml). Infection of transgenic tobacco plants expressing glucose oxidase with R. solani.

Seedlings from several of the tobacco plants found to express glucose oxidases (GOS-9, 13, 24 and GOT-9, 10, 21) and seedlings from a 35SGUS control were surface sterilised and germinated on growth media containing kanamycin. Three weeks later, seedlings homozygous or hemizygous for the kanamycin resistance gene were transferred to sand infested with R. solani to determine their susceptibility to fungal attack. As a control, seedlings were also transferred to sand containing no R. solani. The sand in both experiments was previously moistened with sterilised Hoagland's solution containing 0.5% glucose, the presence of glucose in the solution was necessary to promote fungal infection. After 38 days seedlings were assessed for fungal infection and surviving seedlings tested for glucose oxidase activity with Kl/starch solution. Seedlings were too small to reisolate fungus from to confirm infection by R. solani but symptoms typical of R. solani infection (rotting of hypocotyl and slow growth) were observed only when seedlings were grown in sand infested with R. solani.

All surviving seedlings except those from 35 GUS tested positive for glucose oxidase activity. When grown in sand under control conditions, 85- 100% of all seedlings survived. When grown in infested sand, only 45% of 35SGUS seedlings survived whereas 65-100% of seedlings producing glucose oxidase survived. The 35SGUS seedlings grown in infested sand weighed on average 47% less than 35SGUS seedlings grown under control conditions (Table 7). Little difference in average seedling weight was observed between glucose oxidase expressing seedlings grown in infested or uninfested sand.

Of the glucose oxidase producing seedlings tested, those from GOT-21 seemed to be most susceptible to fungal infection. Only 65% of the seedlings survived when grown in infested sand and the weight of these seedlings on average was slightly lower (80%) than the weight of GOT-21 seedlings grown under control conditions. No significant difference in weight and percentage survival was found among the other glucose oxidase producing seedlings tested. As GOT-21 produces the least amount of glucose oxidase among the transformants tested, this suggests there is a correlation between the level of glucose oxidase activity and resistance to R. solani.

TABLE 7 Average fresh weight of surviving transgenic seedlings after 38 days growth in sand either infested or uninfested with R. solani (4x10⁸ propagules/tray). Twenty seedlings from each transformant were planted in the experiment.

Seedlings Average weight of surviving Infected seedlings weight as a seedlings (g) percentage of control seedlings weight.

Control 4.0x10⁸ R.solani (No. R.solani) propagules/tray

35SGUS 0.089 0.047 53

GOS-9 0.081 0.082 101

GOS-13 0.082 0.090 110

GOS-24 0.110 0.103 94

GOT-9 0.086 0.094 109

GOT-10 0.120 0.110 92

GOT-21 0.085 0.068 80

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Claims

CLAIMS:

1. A genetic construct comprising an isolated nucleotide sequence encoding, or complementary to a sequence encoding, the enzyme glucose oxidase or a functional derivative thereof, said nucleotide sequence being operably linked to a promoter capable of expression in a host organism.

2. A genetic construct according to claim 1 , wherein said nucleotide sequence is operably linked to a promoter capable of expression in a plant cell.

3. A genetic construct according to claim 2, wherein said promoter is capable of expression in cotton.

4. A genetic construct according to claim 2, wherein said promoter is a root specific or inducible promoter.

5. A genetic construct according to claim 4, wherein the promoter is selected from the root-specific pTOBRB7 promoter and the inducible extensin carrot root promoter.

6. A genetic construct according to claim 1 , wherein said nucleotide sequence encodes, or is complementary to a sequence encoding, the glucose oxidase enzyme of Talaromyces flavus or a functional derivative thereof.

7. A genetic construct according to claim 6, wherein said nucleotide sequence corresponds substantially to, or is complementary to, the T. flavus glucose oxidase gene as set out in SEQ. ID NO:1 , or a portion thereof encoding a functional derivative of the glucose oxidase enzyme of 7. flavus.

8. A genetic construct according to claim 6 or claim 7, which includes a signal sequence which expresses functional glucose oxidase enzyme in plant cells.

9. A genetic construct according to claim 8, wherein the signal sequence is the signal sequence of the carrot root extensin gene.

10. A vector molecule comprising a genetic construct according to claim 1.

11. A host organism having integrated therein a vector molecule according to claim 10.

12. A host organism according to claim 11 , which is a plant, a plant cell or a group of cells.

13. A host organism according to claim 12, which is a cotton plant or a cell or a group of cells thereof.

14. A host organism according to claim 11 which is a microorganism or a virus.

15. A host organism according to claim 14, which is a root- or leaf-colonising microorganism or an insect-specific virus.

16. A transgenic organism capable of expressing a cloned nucleotide sequence encoding the enzyme glucose oxidase or a functional derivative thereof.

17. A transgenic organism according to claim 16, which is a plant, a plant cell or a group of plant cells.

18. A transgenic organism according to claim 17, which is a cotton plant or a cell or a group of cells thereof.

19. A transgenic microorganism according to claim 16, which is a microorganism or a virus.

20. A transgenic organism according to claim 19, which is a root- or leaf- colonising microorganism or an insect-specific virus.

21. A method of reducing susceptibility or increasing resistance of a host organism to pests or diseases, which comprises transforming the host organism with a genetic construct according to any one of claims 1 to 9, or a vector molecule according to claim 10.

22. A method according to claim 21, wherein said host organism is a cotton plant or a cell or group of cells thereof.

23. A method of reducing susceptibility or increasing resistance of a host plant to pests or diseases, which comprises transforming a microorganism which colonises the roots or leaves of said host plant, or are insect- specific virus, with a genetic construct according to any one of claims 1 to 9, or a vector molecule according to claim 10.